INSERM U1051, Institut des Neurosciences de Montpellier (INM), Université de Montpellier 1 and 2, Montpellier, France.
Nat Protoc. 2014 May;9(5):1160-9. doi: 10.1038/nprot.2014.073. Epub 2014 Apr 24.
The myelin sheath is essential for the rapid and efficient propagation of action potentials. However, our understanding of the basic molecular mechanisms that regulate myelination, demyelination and remyelination is limited. Schwann cells produce myelin in the peripheral nervous system and remain associated with the axons of peripheral neurons throughout axonal migration to the target. Owing to the intimate relationship between these cell types it is difficult to fully reproduce their function in vitro. For this reason, we developed an approach based on the injection of an engineered virus into the sciatic nerve of mice to locally transduce peripheral nerve cells. This approach can be used as an alternative to germline transgenesis to facilitate the investigation of peripheral nerve biology in vivo. The detailed protocol, described here, requires 3 weeks to complete. In comparison with genetic modification strategies, this protocol is a fast, reproducible and straightforward method for introducing exogenous factors into myelinating Schwann cells and myelinated axons in vivo to investigate specific molecular mechanisms.
髓鞘对于动作电位的快速、有效传播至关重要。然而,我们对调节髓鞘形成、脱髓鞘和髓鞘再生的基本分子机制的理解是有限的。施万细胞在周围神经系统中产生髓鞘,并在轴突向靶器官迁移的过程中始终与周围神经元的轴突相关联。由于这些细胞类型之间的密切关系,很难在体外完全复制它们的功能。基于这一原因,我们开发了一种基于向小鼠坐骨神经注射工程病毒的方法,以局部转导周围神经细胞。这种方法可以替代生殖系基因转移,以促进体内周围神经生物学的研究。这里描述的详细方案需要 3 周时间才能完成。与遗传修饰策略相比,该方案是一种快速、可重复且简单的方法,可将外源性因子引入体内的髓鞘形成施万细胞和髓鞘化轴突中,以研究特定的分子机制。
